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人乳头瘤病毒31型主要衣壳蛋白上中和性构象表位的鉴定及其功能意义

Identification of neutralizing conformational epitopes on the human papillomavirus type 31 major capsid protein and functional implications.

作者信息

Fleury Maxime J J, Touzé Antoine, Maurel Marie-Christine, Moreau Thierry, Coursaget Pierre

机构信息

INSERM U618, Université François Rabelais, Tours, France.

出版信息

Protein Sci. 2009 Jul;18(7):1425-38. doi: 10.1002/pro.156.

Abstract

The aim of this study was to characterize the conformational neutralizing epitopes of the major capsid protein of human papillomavirus type 31. Analysis of the epitopes was performed by competitive epitope mapping using 15 anti-HPV31 and by reactivity analysis using a HPV31 mutant with an insertion of a seven-amino acid motif within the FG loop of the capsid protein. Fine mapping of neutralizing conformational epitopes on HPV L1 was analyzed by a new approach using a system displaying a combinatorial library of constrained peptides exposed on E. coli flagella. The findings demonstrate that the HPV31 FG loop is dense in neutralizing epitopes and suggest that HPV31 MAbs bind to overlapping but distinct epitopes on the central part of the FG loop, in agreement with the exposure of the FG loop on the surface of HPV VLPs, and thus confirming that neutralizing antibodies are mainly located on the tip of capsomeres. In addition, we identified a crossreacting and partially crossneutralizing conformational epitope on the relatively well conserved N-terminal part of the FG loop. Moreover, our findings support the hypothesis that there is no correlation between neutralization and the ability of MAbs to inhibit VLP binding to heparan sulfate, and confirm that the blocking of virus attachment to the extracellular matrix is an important mechanism of neutralization.

摘要

本研究的目的是表征人乳头瘤病毒31型主要衣壳蛋白的构象中和表位。通过使用15种抗HPV31抗体进行竞争性表位图谱分析以及使用一种在衣壳蛋白FG环内插入七氨基酸基序的HPV31突变体进行反应性分析来进行表位分析。通过一种新方法对HPV L1上的中和构象表位进行精细图谱分析,该方法使用一个展示暴露于大肠杆菌鞭毛上的受限肽组合文库的系统。研究结果表明,HPV31的FG环富含中和表位,并且表明HPV31单克隆抗体结合于FG环中部重叠但不同的表位,这与FG环在HPV病毒样颗粒表面的暴露情况一致,从而证实中和抗体主要位于衣壳粒的顶端。此外,我们在FG环相对保守的N端部分鉴定出一个交叉反应且部分交叉中和的构象表位。而且,我们的研究结果支持以下假说:中和作用与单克隆抗体抑制病毒样颗粒与硫酸乙酰肝素结合的能力之间不存在相关性,并证实阻断病毒与细胞外基质的附着是一种重要的中和机制。

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